Use of thiol-terminal silanes and heterobifunctional crosslinkers for immobilization of antibodies on silica surfaces

A procedure for covalent immobilization of functional proteins on silica substrates was developed using thiol-terminal silanes and heterobifunctional crosslinkers. Using this procedure, a high density of functional antibodies was bound to glass cover slips and silica fibers. The amount of anti-IgG a...

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Veröffentlicht in:Analytical biochemistry 1989-05, Vol.178 (2), p.408-413
Hauptverfasser: Bhatia, Suresh K., Shriver-Lake, Lisa C., Prior, Kimberly J., Georger, Jacque H., Calvert, Jeffrey M., Bredehorst, Reinhard, Ligler, Frances S.
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Sprache:eng
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Zusammenfassung:A procedure for covalent immobilization of functional proteins on silica substrates was developed using thiol-terminal silanes and heterobifunctional crosslinkers. Using this procedure, a high density of functional antibodies was bound to glass cover slips and silica fibers. The amount of anti-IgG antibody immobilized was determined to be in the range of 0.66 to 0.96 ng/mm 2 using radiolabeled antibody. The relative amount of IgG antigen bound by the immobilized antibody (0.37 to 0.55 mol antigen/mol antibody) was three to five times greater than other investigators have reported. In addition, the amount of protein nonspecifically adsorbed to the antibody-coated surface was further reduced by the addition of blocking agents so that nonspecific adsorption of protein antigens represented only 2–6% of the total antigen binding. With this low background, IgG antigen binding could be measured at levels as low as 150 fmol when an antigen concentration of 3 pmol/ml was applied. The process for antibody immonilization is straightforward, easy to perform, and adaptable for modifying mass quantities of biosensor components.
ISSN:0003-2697
1096-0309
DOI:10.1016/0003-2697(89)90662-3